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Active-Site Residues of Escherichia coli DNA Gyrase Required in Coupling ATP Hydrolysis to DNA Supercoiling and Amino Acid Substitutions Leading to Novobiocin Resistance

Gross, Christian H. ; Parsons, Jonathan D. ; Grossman, Trudy H. ; [et al.]

American Society for Microbiology ; 2003

In: Antimicrobial Agents and Chemotherapy Vol. 47, No. 3 ( 2003-03), p. 1037-1046

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In: Antimicrobial Agents and Chemotherapy, American Society for Microbiology, Vol. 47, No. 3 ( 2003-03), p. 1037-1046

Abstract: DNA gyrase is a bacterial type II topoisomerase which couples the free energy of ATP hydrolysis to the introduction of negative supercoils into DNA. Amino acids in proximity to bound nonhydrolyzable ATP analog (AMP · PNP) or novobiocin in the gyrase B (GyrB) subunit crystal structures were examined for their roles in enzyme function and novobiocin resistance by site-directed mutagenesis. Purified Escherichia coli GyrB mutant proteins were complexed with the gyrase A subunit to form the functional A 2 B 2 gyrase enzyme. Mutant proteins with alanine substitutions at residues E42, N46, E50, D73, R76, G77, and I78 had reduced or no detectable ATPase activity, indicating a role for these residues in ATP hydrolysis. Interestingly, GyrB proteins with P79A and K103A substitutions retained significant levels of ATPase activity yet demonstrated no DNA supercoiling activity, even with 40-fold more enzyme than the wild-type enzyme, suggesting that these amino acid side chains have a role in the coupling of the two activities. All enzymes relaxed supercoiled DNA to the same extent as the wild-type enzyme did, implying that only ATP-dependent reactions were affected. Mutant genes were examined in vivo for their abilities to complement a temperature-sensitive E. coli gyrB mutant, and the activities correlated well with the in vitro activities. We show that the known R136 novobiocin resistance mutations bestow a significant loss of inhibitor potency in the ATPase assay. Four new residues (D73, G77, I78, and T165) that, when changed to the appropriate amino acid, result in both significant levels of novobiocin resistance and maintain in vivo function were identified in E. coli .

Type of Medium: Online Resource

ISSN: 0066-4804 , 1098-6596

URL: Article

DOI: 10.1128/AAC.47.3.1037-1046.2003

RVK:

XA 24552

Language: English

Publisher: American Society for Microbiology

Publication Date: 2003

detail.hit.zdb_id: 1496156-8

SSG: 12

SSG: 15,3

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Use of Matrix-Assisted Laser Desorption Ionization–Time of Flight Mass Spectrometry To Identify Vancomycin-Resistant Enterococci and Investigate the Epidemiology of an Outbreak

Griffin, Paul M. ; Price, Gareth R. ; Schooneveldt, Jacqueline M. ; [et al.]

American Society for Microbiology ; 2012

In: Journal of Clinical Microbiology Vol. 50, No. 9 ( 2012-09), p. 2918-2931

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In: Journal of Clinical Microbiology, American Society for Microbiology, Vol. 50, No. 9 ( 2012-09), p. 2918-2931

Abstract: The control of vancomycin-resistant enterococci (VRE) has become an increasing burden on health care resources since their discovery over 20 years ago. Current techniques employed for their detection include time-consuming and laborious phenotypic methods or molecular methods requiring costly equipment and consumables and highly trained staff. An accurate, rapid diagnostic test has the ability to greatly reduce the spread of this organism, which has the ability to colonize patients for long periods, potentially even lifelong. Matrix-assisted laser desorption ionization–time of flight mass spectrometry (MALDI-TOF MS) is a technology with the ability to identify organisms in seconds and has shown promise in the identification of other forms of antimicrobial resistance in other organisms. Here we show that MALDI-TOF MS is capable of rapidly and accurately identifying vanB -positive Enterococcus faecium VRE from susceptible isolates. Internal validation of the optimal model generated produced a sensitivity of 92.4% and a specificity of 85.2%. Prospective validation results, following incorporation into the routine laboratory work flow, demonstrated a greater sensitivity and specificity at 96.7% and 98.1%, respectively. In addition, the utilization of MALDI-TOF MS to determine the relatedness of isolates contributing to an outbreak is also demonstrated.

Type of Medium: Online Resource

ISSN: 0095-1137 , 1098-660X

URL: Article

DOI: 10.1128/JCM.01000-12

RVK:

XA 10000

Language: English

Publisher: American Society for Microbiology

Publication Date: 2012

detail.hit.zdb_id: 1498353-9

SSG: 12

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Detection and Characterization of Mycoplasma pneumoniae during an Outbreak of Respiratory Illness at a University

Waller, Jessica L. ; Diaz, Maureen H. ; Petrone, Brianna L. ; [et al.]

American Society for Microbiology ; 2014

In: Journal of Clinical Microbiology Vol. 52, No. 3 ( 2014-03), p. 849-853

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In: Journal of Clinical Microbiology, American Society for Microbiology, Vol. 52, No. 3 ( 2014-03), p. 849-853

Abstract: An outbreak at a university in Georgia was identified after 83 cases of probable pneumonia were reported among students. Respiratory specimens were obtained from 21 students for the outbreak investigation. The TaqMan array card (TAC), a quantitative PCR (qPCR)-based multipathogen detection technology, was used to initially identify Mycoplasma pneumoniae as the causative agent in this outbreak. TAC demonstrated 100% diagnostic specificity and sensitivity compared to those of the multiplex qPCR assay for this agent. All M. pneumoniae specimens ( n = 12) and isolates ( n = 10) were found through genetic analysis to be susceptible to macrolide antibiotics. The strain diversity of M. pneumoniae associated with this outbreak setting was identified using a variety of molecular typing procedures, resulting in two P1 genotypes (types 1 [60%] and 2 [40%] ) and seven different multilocus variable-number tandem-repeat analysis (MLVA) profiles. Continued molecular typing of this organism, particularly during outbreaks, may enhance the current understanding of the epidemiology of M. pneumoniae and may ultimately lead to a more effective public health response.

Type of Medium: Online Resource

ISSN: 0095-1137 , 1098-660X

URL: Article

DOI: 10.1128/JCM.02810-13

RVK:

XA 10000

Language: English

Publisher: American Society for Microbiology

Publication Date: 2014

detail.hit.zdb_id: 1498353-9

SSG: 12

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Immune Restoration Diseases Reflect Diverse Immunopathological Mechanisms

Price, Patricia ; Murdoch, David M. ; Agarwal, Upasna ; [et al.]

American Society for Microbiology ; 2009

In: Clinical Microbiology Reviews Vol. 22, No. 4 ( 2009-10), p. 651-663

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In: Clinical Microbiology Reviews, American Society for Microbiology, Vol. 22, No. 4 ( 2009-10), p. 651-663

Abstract: Up to one in four patients infected with human immunodeficiency virus type 1 and given antiretroviral therapy (ART) experiences inflammatory or cellular proliferative disease associated with a preexisting opportunistic infection, which may be subclinical. These immune restoration diseases (IRD) appear to result from the restoration of immunocompetence. IRD associated with intracellular pathogens are characterized by cellular immune responses and/or granulomatous inflammation. Mycobacterial and cryptococcal IRD are attributed to a pathological overproduction of Th1 cytokines. Clinicopathological characteristics of IRD associated with viral infections suggest different pathogenic mechanisms. For example, IRD associated with varicella-zoster virus or JC polyomavirus infection correlate with a CD8 T-cell response in the central nervous system. Exacerbations or de novo presentations of hepatitis associated with hepatitis C virus (HCV) infection following ART may also reflect restoration of pathogen-specific immune responses as titers of HCV-reactive antibodies rise in parallel with liver enzymes and plasma markers of T-cell activation. Correlations between immunological parameters assessed in longitudinal sample sets and clinical presentations are required to illuminate the diverse immunological scenarios described collectively as IRD. Here we present salient clinical features and review progress toward understanding their pathogeneses.

Type of Medium: Online Resource

ISSN: 0893-8512 , 1098-6618

URL: Article

DOI: 10.1128/CMR.00015-09

RVK:

XA 36863

Language: English

Publisher: American Society for Microbiology

Publication Date: 2009

detail.hit.zdb_id: 1497041-7

SSG: 12

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Molecular Differentiation of Renibacterium salmoninarum Isolates from Worldwide Locations

Grayson, Thomas H. ; Cooper, Lynne F. ; Atienzar, Franck A. ; [et al.]

American Society for Microbiology ; 1999

In: Applied and Environmental Microbiology Vol. 65, No. 3 ( 1999-03), p. 961-968

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In: Applied and Environmental Microbiology, American Society for Microbiology, Vol. 65, No. 3 ( 1999-03), p. 961-968

Abstract: Renibacterium salmoninarum is a genospecies that is an obligate pathogen of salmonid fish and is capable of intracellular survival. Conventional typing systems have failed to differentiate isolates of R. salmoninarum . We used two methods to assess the extent of molecular variation which was present in isolates from different geographic locations. In one analysis we investigated possible polymorphisms in a specific region of the genome, the intergenic spacer (ITS) region between the 16S and 23S rRNA genes. In the other analysis we analyzed differences throughout the genome by using randomly amplified polymorphic DNA (RAPD). We amplified the spacer region of 74 isolates by using PCR and performed a DNA sequence analysis with 14 geographically distinct samples. The results showed that the 16S-23S ribosomal DNA spacer region of R. salmoninarum is highly conserved and suggested that only a single copy of the rRNA operon is present in this slowly growing pathogen. DNA sequencing of the spacer region showed that it was the same length in all 14 isolates examined, and the same nucleotide sequence, sequevar 1, was obtained for 11 of these isolates. Two other sequevars were found. No tRNA genes were found. We found that RAPD analysis allows reproducible differentiation between isolates of R. salmoninarum obtained from different hosts and different geographic regions. By using RAPD analysis it was possible to differentiate between isolates with identical ITS sequences.

Type of Medium: Online Resource

ISSN: 0099-2240 , 1098-5336

URL: Article

DOI: 10.1128/AEM.65.3.961-968.1999

RVK:

WA 15000

Language: English

Publisher: American Society for Microbiology

Publication Date: 1999

detail.hit.zdb_id: 223011-2

detail.hit.zdb_id: 1478346-0

SSG: 12

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Germination-Induced Bioluminescence, a Route To Determine the Inhibitory Effect of a Combination Preservation Treatment on Bacterial Spores

Ciarciaglini, Gianni ; Hill, Philip J. ; Davies, Ken ; [et al.]

American Society for Microbiology ; 2000

In: Applied and Environmental Microbiology Vol. 66, No. 9 ( 2000-09), p. 3735-3742

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In: Applied and Environmental Microbiology, American Society for Microbiology, Vol. 66, No. 9 ( 2000-09), p. 3735-3742

Abstract: In this work, we have used spores of Bacillus subtilis that specifically induce bioluminescence upon initiation of germination as a rapid, real-time monitor of the effects of preservative treatments on germination. Using this tool, we have demonstrated that the combination of mild acidity (pH 5.5 to 5.0), lactic acid (0.5%), and a pasteurization step (90°C for 5 min) results in enhanced inhibition of spore germination compared with the effects of the individual treatments alone. Inhibition by the combination treatment occurred as a result of both direct but reversible inhibition, entirely dependent on the physical presence of the preservative factors, and permanent, nonreversible damage to the l -alanine germination apparatus of the spore. However, we were able to restore germination of the preservative-damaged spores unable to germinate on l -alanine by supplementing the medium with the nonnutrient germinant calcium dipicolinic acid. The demonstration that simple combinations of preservative factors inhibit spore germination indicates that food preservation systems providing ambient stability could be designed which do not adhere to the strict limits set by commonly accepted processes and which are based on precise understanding of their inhibitory action.

Type of Medium: Online Resource

ISSN: 0099-2240 , 1098-5336

URL: Article

DOI: 10.1128/AEM.66.9.3735-3742.2000

RVK:

WA 15000

Language: English

Publisher: American Society for Microbiology

Publication Date: 2000

detail.hit.zdb_id: 223011-2

detail.hit.zdb_id: 1478346-0

SSG: 12

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In Vitro Responsiveness of γδ T Cells from Mycobacterium bovis -Infected Cattle to Mycobacterial Antigens: Predominant Involvement of WC1 + Cells

Smyth, Allister J. ; Kaufmann, S. H. E. ; Welsh, Michael D. ; [et al.]

American Society for Microbiology ; 2001

In: Infection and Immunity Vol. 69, No. 1 ( 2001-01), p. 89-96

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In: Infection and Immunity, American Society for Microbiology, Vol. 69, No. 1 ( 2001-01), p. 89-96

Abstract: It is generally accepted that protective immunity against tuberculosis is generated through the cell-mediated immune (CMI) system, and a greater understanding of such responses is required if better vaccines and diagnostic tests are to be developed. γδ T cells form a major proportion of the peripheral blood mononuclear cells (PBMC) in the ruminant system and, considering data from other species, may have a significant role in CMI responses in bovine tuberculosis. This study compared the in vitro responses of αβ and γδ T cells from Mycobacterium bovis -infected and uninfected cattle. The results showed that, following 24 h of culture of PBMC with M. bovis -derived antigens, the majority of γδ T cells from infected animals became highly activated (upregulation of interleukin-2R), while a lower proportion of the αβ T-cell population showed activation. Similar responses were evident to a lesser degree in uninfected animals. Study of the kinetics of this response showed that γδ T cells remained significantly activated for at least 7 days in culture, while activation of αβ T cells declined during that period. Subsequent analysis revealed that the majority of activated γδ T cells expressed WC1, a 215-kDa surface molecule which is not expressed on human or murine γδ T cells. Furthermore, in comparison with what was found for CD4 + T cells, M. bovis antigen was found to induce strong cellular proliferation but relatively little gamma interferon release by purified WC1 + γδ T cells. Overall, while the role of these cells in protective immunity remains unclear, their highly activated status in response to M. bovis suggests an important role in antimycobacterial immunity, and the ability of γδ T cells to influence other immune cell functions remains to be elucidated, particularly in relation to CMI-based diagnostic tests.

Type of Medium: Online Resource

ISSN: 0019-9567 , 1098-5522

URL: Article

DOI: 10.1128/IAI.69.1.89-96.2001

RVK:

XA 10000

Language: English

Publisher: American Society for Microbiology

Publication Date: 2001

detail.hit.zdb_id: 1483247-1

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